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细胞因子、极性蛋白以及内体蛋白运输与信号传导——体外作为研究模型的支持细胞血睾屏障系统

Cytokines, polarity proteins, and endosomal protein trafficking and signaling-the sertoli cell blood-testis barrier system in vitro as a study model.

作者信息

Xiao Xiang, Wong Elissa W P, Lie Pearl P Y, Mruk Dolores D, Wong Chris K C, Cheng C Yan

机构信息

The Mary M. Wohlford Laboratory for Male Contraceptive Research, Center for Biomedical Research, Population Council, New York, USA; Department of Reproductive Physiology, Zhejiang Academy of Medical Sciences, Hangzhou, Zhejiang, China.

The Mary M. Wohlford Laboratory for Male Contraceptive Research, Center for Biomedical Research, Population Council, New York, USA.

出版信息

Methods Enzymol. 2014;534:181-94. doi: 10.1016/B978-0-12-397926-1.00010-X.

Abstract

Endosomal signaling is emerging as one of the most important cellular events that regulate signaling function in mammalian cells or an epithelium in response to changes in environment such as the presence of stimuli mediated by cytokines, toxicants, heat, ions during growth and development, and other cellular processes such as cytokinesis and spermatogenesis. Recent studies have shown that protein endocytosis-the initial step of endosomal signaling-involves the participation of polarity proteins, such as partitioning defective protein 6 (Par6), Cdc42 and 14-3-3 (also known as Par5), which in turn is regulated by cytokines (e.g., TGF-β2, TGF-β3) and testosterone at the Sertoli cell blood-testis barrier (BTB) in the mammalian testis. In this short method paper, we provide a detailed protocol of assessing protein endocytosis, the initial and also the most critical step of endosomal signaling at the Sertoli cell BTB. This biochemical endocytosis assay summarizes our experience for the last decade, which should likely be performed in conjunction with the dual-labeled immunofluorescence analysis to assess protein endocytosis. While we are using a Sertoli cell in vitro system that mimics the BTB in vivo, this approach should be applicable to virtually all mammalian cells.

摘要

内体信号传导正成为最重要的细胞事件之一,它在哺乳动物细胞或上皮细胞中调节信号功能,以响应环境变化,如细胞因子、毒物、热、生长发育过程中的离子等介导的刺激,以及其他细胞过程,如胞质分裂和精子发生。最近的研究表明,蛋白质内吞作用——内体信号传导的起始步骤——涉及极性蛋白的参与,如分区缺陷蛋白6(Par6)、Cdc42和14-3-3(也称为Par5),而这些蛋白又受到细胞因子(如TGF-β2、TGF-β3)和哺乳动物睾丸支持细胞血睾屏障(BTB)处的睾酮的调节。在这篇简短的方法论文中,我们提供了一个详细的方案,用于评估蛋白质内吞作用,这是支持细胞BTB处内体信号传导的起始且最为关键的步骤。这种生化内吞作用测定总结了我们过去十年的经验,应该与双标记免疫荧光分析一起进行,以评估蛋白质内吞作用。虽然我们使用的是体外模拟体内BTB的支持细胞系统,但这种方法几乎适用于所有哺乳动物细胞。

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